Literature DB >> 12432067

Lasp-1 binds to non-muscle F-actin in vitro and is localized within multiple sites of dynamic actin assembly in vivo.

Catherine S Chew1, Xunsheng Chen, John A Parente, Shannan Tarrer, Curtis Okamoto, Hai-Yen Qin.   

Abstract

Lasp-1 has been identified as a signaling molecule that is phosphorylated upon elevation of [cAMP]i in pancreas, intestine and gastric mucosa and is selectively expressed in cells within epithelial tissues. In the gastric parietal cell, cAMP-dependent phosphorylation induces the partial translocation of lasp-1 to the apically directed F-actin-rich canalicular membrane, which is the site of active HCl secretion. Lasp-1 is an unusual modular protein that contains an N-terminal LIM domain, a C-terminal SH3 domain and two internal nebulin repeats. Domain-based analyses have recently categorized this protein as an epithelial representative of the nebulin family, which also includes the actin binding, muscle-specific proteins, nebulin, nebulette and N-RAP. In this study, we show that lasp-1 binds to non-muscle filamentous (F) actin in vitro in a phosphorylation-dependent manner. In addition, we provide evidence that lasp-1 is concentrated within focal complexes as well as in the leading edges of lamellipodia and the tips of filopodia in non-transformed gastric fibroblasts. In actin pull-down assays, the apparent K(d) of bacterially expressed his-tagged lasp-1 binding to F-actin was 2 micro M with a saturation stoichiometry of approximately 1:7. Phosphorylation of recombinant lasp-1 with recombinant PKA increased the K(d) and decreased the B(max) for lasp-1 binding to F-actin. Microsequencing and site-directed mutagenesis localized the major in vivo and in vitro PKA-dependent phosphorylation sites in rabbit lasp-1 to S(99) and S(146). BLAST searches confirmed that both sites are conserved in human and chicken homologues. Transfection of lasp-1 cDNA encoding for alanine substitutions at S(99) and S(146), into parietal cells appeared to suppress the cAMP-dependent translocation of lasp-1 to the intracellular canalicular region. In gastric fibroblasts, exposure to the protein kinase C activator, PMA, was correlated with the translocation of lasp-1 into newly formed F-actin-rich lamellipodial extensions and nascent focal complexes. Since lasp-1 does not appear to be phosphorylated by PKC, these data suggest that other mechanisms in addition to cAMP-dependent phosphorylation can mediate the translocation of lasp-1 to regions of dynamic actin turnover. The localization of lasp-1 to these subcellular regions under a range of experimental conditions and the phosphorylation-dependent regulation of this protein in F-actin rich epithelial cells suggests an integral and possibly cell-specific role in modulating cytoskeletal/membrane-based cellular activities.

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Year:  2002        PMID: 12432067     DOI: 10.1242/jcs.00174

Source DB:  PubMed          Journal:  J Cell Sci        ISSN: 0021-9533            Impact factor:   5.285


  47 in total

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Review 2.  Regulation of Transporters and Channels by Membrane-Trafficking Complexes in Epithelial Cells.

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5.  Ectopic expression of LIM-nebulette (LASP2) reveals roles in cell migration and spreading.

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7.  Nuclear localisation of LASP-1 correlates with poor long-term survival in female breast cancer.

Authors:  J J Frietsch; T G P Grunewald; S Jasper; U Kammerer; S Herterich; M Kapp; A Honig; E Butt
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9.  Lasp1 gene disruption is linked to enhanced cell migration and tumor formation.

Authors:  Han Zhang; Xunsheng Chen; Wendy B Bollag; Roni J Bollag; Daniel J Sheehan; Catherine S Chew
Journal:  Physiol Genomics       Date:  2009-06-16       Impact factor: 3.107

10.  Contribution of the LIM domain and nebulin-repeats to the interaction of Lasp-2 with actin filaments and focal adhesions.

Authors:  Hiroyuki Nakagawa; Hiroshi Suzuki; Satoshi Machida; Junko Suzuki; Kazuyo Ohashi; Mingyue Jin; Shigeaki Miyamoto; Asako G Terasaki
Journal:  PLoS One       Date:  2009-10-23       Impact factor: 3.240

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